Association of Dominant and Recessive Genes Confers Anthracnose Resistance in Stem and Leaves of Common Bean

Different genes might be involved in Colletotrichum lindemuthianum resistance in leaves and stem of common bean. This work aimed to study the genetic mechanisms of the resistance in the leaf and stem in segregating populations from backcrosses involving resistant cultivar AN 910408 and susceptible cultivar Rudá inoculated with spore suspensions of C. lindemuthianum race 83. Our results indicate that two genes which interact epistatically, one dominant and one recessive, are involved in the genetic control of leaf anthracnose resistance. As for stem anthracnose resistance, two genes also epistatic, one dominant and one recessive, explain the resistance to C. lindemuthianum race 83. The recessive gene is the same for leaf and stem resistance; however, the dominant genes are distinct and independent from each other. The three independent resistance genes of AN 910408 observed in this work could be derived from Guanajuato 31.     

Sources of Resistance to Anthracnose in Traditional Common Bean Cultivars from Paraná, Brazil

Pathogenicity of physiologically distinct races of Colletotrichum lindemuthianum originating from Andean (races 7, 19 and 55) and Mesoamerican (races 9, 31, 65, 69, 73, 81, 89, 95 and 453) locations of the new world were evaluated on 26 landrace genotypes of common bean (Phaseolus vulgaris L.) from Paraná State, Brazil. Races 7 (Andean), 65, 73 and 89 (Mesoamerican) were the most pathogenic, while race 31 (Mesoamerican) was the least pathogenic. Most of the landrace genotypes evaluated (88%) were resistant to race 31, except Carioca 3, Preto 1 and Preto 2. In addition, about 50% of the landrace genotypes had resistance to races 9, 19, 55 and 453; and about 30% to races 7, 65, 69, 73, 81, 89 and 95. The resistance index, which measured the pathogenicity response averaged across all the physiologically distinct Andean and Mesoamerican races of C. lindemuthianum, of the landrace genotypes ranged from 8% to 83%. The most resistant cultivars were Carioca Pintado 1, Carioca Pintado 2, Jalo Vermelho and Jalo de Listras Pretas. In contrast, the most susceptible cultivars were Jalo Pardo, Jalo Pintado 1 and Bolinha that showed resistance only to the least pathogenic race 31. These results indicated that many of the common bean landrace cultivars evaluated have genes that could be useful in breeding programmes to enhance resistance to Andean and Mesoamerican races of C. lindemuthianum.     

Allelism Tests between the Rust Resistance Gene Present in Common Bean Cultivar Ouro Negro and Genes Ur-5 and Ur-11

The pathogenic variability of the fungus Uromyces appendiculatus is an obstacle for the creation of rust‐resistant common bean (Phaseolus vulgaris L.) varieties. Gene pyramiding is an alternative strategy for the development of varieties with durable resistance. However, to reach this goal it is important to identify different genes with ample resistance spectra. Cultivars Ouro Negro, Mexico 309 and Belmidak RR‐3 have been shown to be resistant to several rust races identified in the state of Minas Gerais, Brazil. Ouro Negro is the only rust resistance source being used in the BIOAGRO/Universidade Federal de Viçosa (UFV) breeding programme, which aims at pyramiding resistance genes in the ‘carioca‐type’ cultivar Rudá. It would be also interesting to use Mexico 309 (Ur‐5) and Belmidak RR‐3 (Ur‐11) in the breeding programme. However, there is no available information on the possible allelic relationships between the Ouro Negro resistance gene and Ur‐5 and Ur‐11. This work aimed at: (1) determining the allelic relationship between the Ouro Negro resistance gene and Ur‐5 and Ur‐11; and (2) evaluating a random amplified polymorphic DNA (RAPD) marker previously reported as being linked to Ur‐11, in populations from crosses between Belmidak RR‐3 and Rudá. The allelism tests confirmed that the Ouro Negro rust resistance gene is distinct from Ur‐5 and Ur‐11 and the molecular analyses confirmed that the RAPD marker can be used in our breeding programme to develop ‘carioca‐type’ cultivars with the Ur‐11 gene.     

普通菜豆抗炭疽病基因鉴定与分子标记

菜豆炭疽病是世界菜豆生产中的主要病害之一,使幕豆产量和品质受到严重影响,对抗炭疽病基因的研究可以为培育抗炭疽病品种奠定基础。幕豆炭疽病病菌生理分化比较复杂,由于菜豆品种的抗病性和地域不同,菜豆炭疽菌的致病性分化不同。10个已知抗炭疽病基因中,9个基因（Co-1、Co-2、Co-3／Co-9、Co-4^2、Co-5、Co-6、Co-7、Co-10）已被确认为独立显性基因,其中Co-3／Co-9是等位基因;Co-1、Co-4和Co-9存在等位基因,co-8为隐性基因。除Co-5、Co-7和co-8三个基因还没有被定位外,其他基因被定位在不同的连锁群上。     

δ 13C of CO2 respired in the dark in relation to δ13C of leaf carbohydrates in Phaseolus vulgaris L. under progressive drought

The variations in δ ¹³C in both leaf carbohydrates (starch and sucrose) and CO₂ respired in the dark from the cotyledonary leaves of Phaseolus vulgaris L. were investigated during a progressive drought. As expected, sucrose and starch became heavier (enriched in ¹³C) with decreasing stomatal conductance and decreasing p _i/ p _a during the first half (15 d) of the dehydration cycle. Thereafter, when stomata remained closed and leaf net photosynthesis was near zero, the tendency was reversed: the carbohydrates became lighter (depleted in ¹³C). This may be explained by increased p _i/ p _a but other possible explanations are also discussed. Interestingly, the variations in δ ¹³C of CO₂ respired in the dark were correlated with those of sucrose for both well-watered and dehydrated plants. A linear relationship was obtained between δ ¹³C of CO₂ respired in the dark and sucrose, respired CO₂ always being enriched in ¹³C compared with sucrose by ≈ 6‰. The whole leaf organic matter was depleted in ¹³C compared with leaf carbohydrates by at least 1‰. These results suggest that: (i) a discrimination by ≈ 6‰ occurs during dark respiration processes releasing ¹³C-enriched CO₂; and that (ii) this leads to ¹³C depletion in the remaining leaf material.     

Utilization of the acetylene reduction assay to screen for tolerance of symbiotic N2 fixation to limiting P nutrition in common bean

The limitation of symbiotic nitrogen fixation due to P deficiency restricts the development of a sustainable agriculture, particularly in Mediterrancan and tropical soils. Common bean genotypes, APN18, BAT271, PVA846, POT51, G2633 and G12168, were grown in an aerated N-free nutrient solution at low (72 μmol plant^-1 week^-1) and control P supplies (360 μmol plant^-1 week^-1). Nitrogenase activity was estimated by in situ measurements of acetylene reduction activity (ARA) in a flow-through system. During the assays, maximum values of ARA (peak ARA) were reached between 20 and 30 min after exposure to C₂H₂, depending on P treatment and growth stage. Thereafter, a decline in C₂H₄ evolution was observed. This decline was most pronounced in low-P plants and there was a significant genotypic effect. ARA per plant was decreased by P deficiency, mostly because nodulation was delayed and the number and mass of nodules were reduced. The ARA decrease during pod filling was also activated by P deficiency. ARA per g dry weight nodule was increased by P deficiency in G2633 and G12168, unchanged in APN18, BAT271 and POT51 and decreased in PVA846. Except for the climbing type IV G2633, total N at harvest for all P treatments was correlated with the cumulative value of peak ARA and with peak ARA at early pod-filling which was the highest peak ARA throughout the growth cycle of type III bushy genotypes. We conclude that if phenology and growth habit are carefully considered, peak ARA is a reliable screen of genotypes for N² fixation tolerance to P deficiency. Selection of lines with early nodulation under P deficiency is also advisable, and the effect of P deficiency on the nodule functioning needs to be considered.     

The vacuolar localization of a basic peroxidase isoenzyme responsible for the synthesis of α-31,41-anhydrovinblastine in Catharanthus roseus (L.) G. Don Leaves

Partially purified protein extracts of Catharanthus roseus leaves were able to couple catharanthine and vindoline to produce α-3′,4′-anhydrovinblastine (AVLB) in a reaction strictly dependent on H₂O₂. This result, and the co-purification of peroxidase with AVLB synthetase activity, strongly suggest a peroxidase-like nature for the coupling enzyme. Only one peroxidase isoenzyme was detected in C. roseus leaves, and it was shown that this isoenzyme consists of a molecularly-heterogeneous basic peroxidase (EC 1-11-1-7) mainly located in the vacuole. These results suggest that a basic peroxidase located in the vacuole may be the main enzyme responsible for AVLB synthesis in C. roseus leaves. This isoenzyme was also found in cell walls where a peroxidase inhibitor was detected.     

Modeling of the Interaction of Na+ and K+ with the Binding of the Cocaine Analogue 3β-(4-[125I]Iodophenyl)tropane-2β-Carboxylic Acid Isopropyl Ester to the Dopamine Transporter

Abstract: The present study examines the interaction of Na⁺ and K⁺ with the binding of the cocaine analogue 3β-(4-[¹²⁵I]iodophenyl)tropane-2β-carboxylic acid isopropyl ester to dopamine transporters (DATs) in rat striatal synaptosomal membranes at 37°C. The binding increases with [Na⁺] from 10 to 100 mM and decreases with higher [Na⁺]. The presence of K⁺ reduces the maximal stimulatory effect of Na⁺ and causes a nonlinear EC₅₀ shift for Na⁺. K⁺ strongly inhibits the binding at low [Na⁺]. Increasing [Na⁺] produces a linear IC₅₀ shift for K⁺. Saturation analysis indicates a single binding site changing its affinity for the radioligand depending on [K⁺]/[Na⁺] ratio in the assay buffer. A reduced B_max was observed in the presence of 10 mM Na⁺ and 30 mM K⁺. Both high [Na⁺] and high [K⁺] accelerate the dissociation of the binding, and K⁺-induced acceleration was abolished by increasing [Na⁺]. Least squares model fitting of equilibrium data and kinetic analysis of dissociation rates reveal competitive interactions between Na⁺ and K⁺ at two sites allosterically linked on the DAT: One site mediates the stimulatory effect of Na⁺, and the other site involves the radioligand binding and the inhibitory effect of cations on the binding. Various uptake blockers and substrates, dopamine in particular, display reduced potency in inhibiting the binding at a higher [K⁺]/[Na⁺] ratio.